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辐射诱导正常人尿路上皮培养物中c-myc癌蛋白表达及细胞增殖。

Induction of c-myc oncoprotein and of cellular proliferation by radiation in normal human urothelial cultures.

作者信息

Mothersill C, Seymour C B, O'Brien A

机构信息

Radiobiology Research Group, Nuclear Energy Board, Dublin, Ireland.

出版信息

Anticancer Res. 1991 Jul-Aug;11(4):1609-12.

PMID:1746918
Abstract

Normal urothelial cultures were established from transplant ureters and irradiated or exposed to nitrosamines. The cells which survived the treatment were monitored for expression of c-myc oncoprotein. The cultures were also exposed to tritiated thymidine (3HTdR) to determine the total number of cells synthesizing DNA. The area of explant outgrowth was also measured. Proliferation is considered to be a fundamental precondition which has to be present before malignant change can take place or which has to accompany this change. The results indicate that the overall growth rate of the carcinogen-treated cultures is relatively faster than that of the controls. This is particularly true one to two weeks after carcinogen exposure. Certain areas of the culture develop abnormally, cells are different in size and shape to the normal uroepithelial cell and have the capacity to pile up and form characteristic foci. These foci continue to proliferate after senescence of control cultures and after senescence of normal areas of treated cultures. The cells in these foci express high levels of c-Myc oncoprotein. Control and treated but normal cells are negative for this antigen under the conditions used. N-ethyl nitrosamine (NEN) (0.005-0.05 micrograms/ml) and radiation (2.5-10.0 Gy) are both able to induce the changes described. The results suggest that radiation and/or nitrosamine treatment can induce uroepithelial cells to divide at a faster rate than usual. Certain cells within this fast growing culture attain the capacity to pile up and acquire a different morphology. These cells do not senescence at the usual time and are c-myc positive. They may represent a subpopulation which has undergone some pre or early malignant changes.

摘要

从移植输尿管建立正常尿路上皮培养物,并对其进行辐射或使其暴露于亚硝胺。对经处理后存活的细胞监测c-myc癌蛋白的表达。培养物还暴露于氚标记的胸腺嘧啶核苷(3HTdR),以确定合成DNA的细胞总数。还测量了外植体生长的面积。增殖被认为是恶性变化发生之前必须存在的基本前提条件,或者是必须伴随这种变化的条件。结果表明,致癌物处理后的培养物总体生长速度比对照培养物相对更快。在致癌物暴露后一到两周尤其如此。培养物的某些区域发育异常,细胞的大小和形状与正常尿路上皮细胞不同,并且有堆积并形成特征性病灶的能力。在对照培养物衰老以及处理过的培养物正常区域衰老后,这些病灶继续增殖。这些病灶中的细胞表达高水平的c-Myc癌蛋白。在所用条件下,对照细胞和经处理但正常的细胞对该抗原呈阴性。N-乙基亚硝胺(NEN)(0.005 - 0.05微克/毫升)和辐射(2.5 - 10.0 Gy)都能够诱导所述变化。结果表明,辐射和/或亚硝胺处理可诱导尿路上皮细胞以比平常更快的速度分裂。在这种快速生长的培养物中的某些细胞获得堆积的能力并获得不同的形态。这些细胞不会在通常时间衰老并且c-myc呈阳性。它们可能代表已经经历了一些前期或早期恶性变化的亚群。

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